Immunogenicity and protective efficacy of an inactivated bivalent vaccine containing two recombinant H1N1 and H3N2 swine influenza virus strains

被引:0
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作者
Heng Zhang [1 ]
Xu Chen [2 ]
Dongying Liu [1 ]
Xinyu Liu [1 ]
Yifan Ge [1 ]
Yani Sun [1 ]
Xiaoyue Zhang [1 ]
Guangen Hao [2 ]
Zhaoyang Li [2 ]
Qingqing Song [2 ]
Lei Wang [2 ]
Zhao Wang [1 ]
Huanliang Yang [5 ]
Qing Pan [4 ]
Qin Zhao [3 ]
机构
[1] Northwest A&F University,College of Veterinary Medicine
[2] Shandong SINDER Technology Co.,Swine Disease R&D Center
[3] Ltd,College of Veterinary Medicine
[4] Qingdao Agricultural University,Key Laboratory of Animal Influenza, Ministry of Agriculture and Rural Affairs
[5] Harbin Veterinary Research Institute,School of Laboratory Animal & Shandong Laboratory Animal Center
[6] Chinese Academy of Agricultural Sciences,undefined
[7] Shandong First Medical University,undefined
[8] Shandong Academy of Medical Sciences,undefined
关键词
Swine influenza virus; H1N1 subtype; H3N2 subtype; Immune duration; Protective efficacy;
D O I
10.1007/s00018-025-05674-0
中图分类号
学科分类号
摘要
The wild-type H1N1 and H3N2 swine influenza virus (SIV) strains are unsuitable for vaccine production because of high lethality in chicken embryos and low reproductive titers. This study developed recombinant H1N1-Re1 and H3N2-Re1 strains via HA and NA genes from the wild-type H1N1 SW/GX/755/17 and H3N2 SW/GX/1659/17 strains combined with six internal genes from the H1N1 A/PR/8/34 strain. The recombinant viruses demonstrated typical cytopathic effects in MDCK cells, and the presence of viral particles was confirmed via electron microscopy. Growth curve analysis revealed titers of 108.31 and 108.17 EID50 per 100 µL for H1N1-Re1 and H3N2-Re1, respectively, within 72–96 h postinoculation. Virus stocks were used to produce a bivalent inactivated vaccine. After two immunizations, hemagglutination inhibition titers in piglets were significantly greater than those induced by commercial vaccines and were sustained from 5 to 29 weeks postimmunization. Upon challenge with virulent wild-type SIV strains, viral isolation occurred in all pigs in the PBS group (5/5 protection), whereas no virus was detected in the bivalent vaccine group (0/5). In contrast, the commercial vaccine group had a viral isolation rate of 1/5. Pathological examination revealed severe pulmonary lesions in the PBS group, mild changes in the commercial vaccine group (1/5), and normal lung morphology in the bivalent vaccine group. This study demonstrated the successful application of an eight-plasmid reverse genetics system to develop recombinant vaccine strains with enhanced immunogenicity and replication efficiency. The bivalent inactivated vaccine provides prolonged and complete protection against H1N1 and H3N2 SIV strains, offering a robust tool for controlling evolving SIV variants.
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